用于口服肽类药物的给药系统 (DDS) 含有促进和增强吸收的赋形剂。然而,关于 DDS 辅料如渗透促进剂如何与胃肠道粘液屏障相互作用的知识很少。本研究旨在研究渗透增强剂 8-[(2-羟基苯甲酰基)氨基]辛酸钠 (SNAC) 与离体猪肠粘液 (PIM)、离体猪胃粘液 (PGM) 以及体外生物仿制药粘液 (BM) 通过分析其暴露于 SNAC 后的物理和屏障特性。使用肽环孢菌素 A 和万古霉素、卵清蛋白作为模型蛋白质以及不同分子量和不同表面电荷的荧光素-异硫氰酸酯葡聚糖 (FD) 进行大量粘液渗透性研究,同时使用质地分析仪进行粘液保留力研究,流变学研究、冷冻扫描电子显微镜 (cryo-SEM) 和荧光标记纳米颗粒的单颗粒跟踪,以研究 SNAC-粘液相互作用的影响。SNAC 暴露于 PIM 增加了粘液保留力、储能模量、粘度,增加了 PIM 内的纳米颗粒限制,并减少了环孢菌素 A 和卵清蛋白通过 PIM 的渗透。出奇,PGM 的粘度以及环孢菌素 A 和卵清蛋白通过 PGM 的渗透不受 SNAC 存在的影响,因此 SNAC 的作用取决于收集粘液的区域部位。在没有 SNAC 的情况下,不同分子量和不同电荷的 FDs 通过 PIM 的渗透与通过 BM 的渗透相当。然而,虽然两种 FD 通过 PIM 的大量渗透都不受 SNAC 的影响,但 SNAC 的存在降低了 FD4 的渗透并增加了 FD150 kDa 通过 BM 的渗透。此外,与 PIM 中的观察结果相反,BM 内的纳米粒子限制不受 SNAC 存在的影响。总之,本研究表明 SNAC 改变了 PIM 的物理和阻隔特性,但没有改变 PGM。在 BM 中未观察到 SNAC 对 PIM 的影响体外模型。总而言之,该研究强调需要进一步了解渗透增强剂如何影响粘液屏障,并说明应谨慎选择用于此类研究的选定粘液模型。
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Physical and barrier changes in gastrointestinal mucus induced by the permeation enhancer sodium 8-[(2-hydroxybenzoyl)amino]octanoate (SNAC)
Drug delivery systems (DDS) for oral delivery of peptide drugs contain excipients that facilitate and enhance absorption. However, little knowledge exists on how DDS excipients such as permeation enhancers interact with the gastrointestinal mucus barrier. This study aimed to investigate interactions of the permeation enhancer sodium 8-[(2-hydroxybenzoyl)amino]octanoate (SNAC) with ex vivo porcine intestinal mucus (PIM), ex vivo porcine gastric mucus (PGM), as well as with in vitro biosimilar mucus (BM) by profiling their physical and barrier properties upon exposure to SNAC. Bulk mucus permeability studies using the peptides cyclosporine A and vancomycin, ovalbumin as a model protein, as well as fluorescein-isothiocyanate dextrans (FDs) of different molecular weights and different surface charges were conducted in parallel to mucus retention force studies using a texture analyzer, rheological studies, cryo-scanning electron microscopy (cryo-SEM), and single particle tracking of fluorescence-labelled nanoparticles to investigate the effects of the SNAC-mucus interaction. The exposure of SNAC to PIM increased the mucus retention force, storage modulus, viscosity, increased nanoparticle confinement within PIM as well as decreased the permeation of cyclosporine A and ovalbumin through PIM. Surprisingly, the viscosity of PGM and the permeation of cyclosporine A and ovalbumin through PGM was unaffected by the presence of SNAC, thus the effect of SNAC depended on the regional site that mucus was collected from. In the absence of SNAC, the permeation of different molecular weight and differently charged FDs through PIM was comparable to that through BM. However, while bulk permeation of neither of the FDs through PIM was affected by SNAC, the presence of SNAC decreased the permeation of FD4 and increased the permeation of FD150 kDa through BM. Additionally, and in contrast to observations in PIM, nanoparticle confinement within BM remained unaffected by the presence of SNAC. In conclusion, the present study showed that SNAC altered the physical and barrier properties of PIM, but not of PGM. The effects of SNAC in PIM were not observed in the BM in vitro model. Altogether, the study highlights the need for further understanding how permeation enhancers influence the mucus barrier and illustrates that the selected mucus model for such studies should be chosen with care.
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